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  • Dampor
    Member
    • Jun 2012
    • 14

    ATAC-seq plasmid contamination after transfection

    HI all

    I am trying to produce ATAC-seq libraries from transfected cells, but it seems a pain...

    I have produced good libraries from non-transfected cells (sequencing was OK), but when I transfect cells with a plasmid I get, of course, a lot of tagmentation in the plasmid, such that most of my reads are plasmid-derived. I would like not to diminish the plasmid concentration, because all my experiment so far have been done using the same conditions.

    We are trying to solve this problem but it does not look easy...

    My idea is to get rid of the plasmid before tagmentation and probably use AMPure beads to suck it up just after lysing the cells. But I am not sure how this will work because there may be complications (I am going to test this next week, I think)

    Another possibility is to check the tagmented genome (before amplification) on a gel and see if it is be possible to separate the plasmid from the genome. This actually raises the question if the genomic DNA is fragmented after tagmentation (I think it is, unfortunately... can you confirm?)

    We were also considering sequence capture to get rid of the plasmid fragments, but this also has some problem in the fact that the adapters may then hybridise together resulting in non specific sequence capture.

    Please let me know if you have found such a problem and came up with a solution.
    Very much appreciated

    Bests
    Dam
  • rbd
    Junior Member
    • Oct 2014
    • 6

    #2
    This isn't something that I have tried but I have thought about it. If your plasmid isn't too long you could possibly try using long biotinylated oligos that will hybridize to known sequence in your plasmid. You then pull down plasmid DNA fragments from your ATACseq sample post-tagmentation, pre-amplification.

    I would be interested to hear other people's thoughts about the viability of such a method.

    Also there is another method which is likely to be more viable since it has already been published. I think there are some papers out using CRISPR/Cas9 and sgRNAs to deplete mitochondrial DNA in ATACseq samples. I don't see why that can't be applied to deplete your plasmid DNA.

    check out this link

    ATAC-seq is a high-throughput sequencing technique that aims at identifying DNA sequences located in open chromatin. Depending on the cell type, ATAC-seq may yield a high number of mitochondrial sequencing reads (∽20-80% of the reads). As the regions of open chromatin of interest are usually located in the nuclear genome, mitochondrial reads are typically discarded from the analysis. To decrease wasted sequencing, we performed targeted cleavage of mitochondrial DNA using CRISPR/Cas9 and 100 mtDNA-specific guide RNAs. We also tested a modified ATAC-seq protocol that does not include detergent in the cell lysis buffer. Both treatments resulted in considerable reduction of mitochondrial reads (1.7 and 3-fold, respectively). The removal of detergent, however, resulted in increased background and fewer peaks identified. The highest number of peaks and highest quality data was obtained by preparing samples with the original ATAC-seq protocol (using detergent) and treating them with anti-mitochondrial guide RNAs and Cas9. This strategy could lead to considerable cost reduction and improved peak calling when performing ATAC-seq on a moderate to large number of samples and in cell types that contain a large amount of mitochondria.


    Also, to answer your question, the DNA is fragmented after tagmentation.

    Comment

    • nucacidhunter
      Jafar Jabbari
      • Jan 2013
      • 1250

      #3
      It might be possible to adapt NuGEN AnyDeplete technology to get rid of plasmid sequences.

      Sequence capture will not work as only one strand of plasmid read will be captured and the other strand will stay in supernatant along the host fragments which will be amplified or sequenced. If you use host probes for capture it might be expensive as probes have to be synthesised for whole host genome.

      Comment

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